Arch Microbiol (2007) 188:367–375
DOI 10.1007/s00203-007-0257-2ORIGINAL PAPER
Characterization of a broad range antibacterial substance from a new Bacillus species isolated from Amazon basin
Amanda S. Motta · Fabiana S. Cannavan · Siu-Mui Tsai · Adriano Brandelli
Received: 5 December 2005 / Revised: 19 January 2007 / Accepted: 17 April 2007 / Published online: 30 May 2007© Springer-Verlag 2007
Abstract A Bacillus sp. strain producing a bacteriocin-like substance was characterized by biochemical proWlingand 16S rDNA sequencing. The phylogenetic analysis indi-cated that this strain has low sequence similarity with mostBacillus spp., suggesting a new species was isolated. Theantimicrobial activity was detected starting at the exponen-tial growth phase, and maximum activity was observed atstationary phase. The substance was inhibitory to a broadrange of indicator strains, incluing pathogenic and foodspoilage bacteria such as Listeria monocytogenes,B. cereus, Aeromonas hydrophila, Erwinia carotovora,Pasteurella haemolytica, Salmonella Gallinarum, amongother. The antibacterial substance was stable over a widepH range, but it was sensitive to pronase E and lipase. Theantibacterial substance was bactericidal and bacteriolytic toL. monocytogenes and B. cereus at 160 AU ml¡1. The iden-tiWcation of a broad range bacteriocin-like inhibitory sub-stance active against L. monocytogenes addresses animportant aspect of food protection against pathogens andspoilage microorganisms.
Keywords Amazon · Antimicrobial · Bacillus · Bacteriocin · Fish bacteria
Introduction
Antimicrobial substances are widespread produced amongbacteria. Bacteriocins and bacteriocin-like inhibitory sub-stances (BLIS) are antimicrobial peptides produced by anumber of diVerent bacteria that are often eVective againstclosely related species (Tagg et al. 1976; Riley and Wertz2002).
Bacteriocins have received increasing attention due totheir potential use as natural preservatives in food industry,as probiotics in the human health, and as therapeutic agentsagainst pathogenic microorganisms (Riley and Wertz2002). Althoug research eVorts are mainly focused on bac-teriocins produced by lactic acid bacteria, bacteriocins froma variety of Gram-positive and Gram-negative species havebeen characterized (Gould 1996; McAuliVe et al. 2001).They can be divided into three major classes of which classI and II are quite heat-stable. Class I contains modiWed bac-teriocins, so-called lantibiotics, that are found amongstmany diVerent Gram-positive bacteria but have yet to befound in Gram-negative bacteria. They are divided into twosubclasses (a) the linear and cationic peptide and (b) theglobular peptides; the latter normally are hydrophobic butnot cationic. The second major class (II) contains smallheat-stable bacteriocins that lack posttranslational modiW-cations as found in lantibiotics, and are presently clusteredinto at least two groups: pediocin-like bacteriocins andtwo-peptide bacteriocins (Diep and Nes 2002). A third class(III) of bacteriocins has been also deWned. They arenormally larger in size and are easily subjected to heatinactivation (Klaenhammer 1993).
The conventional wisdom about the killing range of bac-teriocins from Gram-positive bacteria is that they arerestricted to killing other Gram-positive bacteria. The rangeof susceptible strains can vary signiWcantly, from relatively
Communicated by Jean-Luc Pernodet.
A. S. Motta · A. Brandelli (&)Laboratório de Bioquímica e Microbiologia Aplicada, Departamento de Ciência de Alimentos, ICTA, Universidade Federal do Rio Grande do Sul, Av. Bento Gonçalves 9500, 91501-970 Porto Alegre, Brazile-mail: [email protected]
F. S. Cannavan · S.-M. TsaiCentro de Energia Nuclear na Agricultura, Universidade de São Paulo, Piracicaba, Brazil
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368 Arch Microbiol (2007) 188:367–375
narrow as in the case of lactococcins A, B and M, whichhave been found to kill only Lactococcus, to extraordinarilybroad (Ross et al. 1999).
Bacillus species are aerobic spore formers commonlyfound in soil and ground water and often encountered onplants and animals at the point of harvest or slaughter.Bacillus is a genus that have been investigated for produc-ing so-called bacteriocin-like inhibitory substance (BLIS)and strains of B. thuringiensis, B. subtilis, B. stearothermo-philus, B. licheniformis, B. megaterium and B. cereus havebeen reported to produce BLIS (Stein 2005; Gray et al. 2006;He et al. 2006; Lisboa et al. 2006; Sharma et al. 2006).
We recently reported antimicrobial activity among severalbacteria isolated from aquatic environments of BrazilianAmazon basin (Motta et al. 2004). The bacterium P34 wasisolated from the Amazonian Wsh Piau-com-pinta as a strainproducing an antimicrobial substance that inhibits the patho-gen Listeria monocytogenes. This antimicrobial substancehas a molecular mass of 1,456 Da, was relatively heat stableand sensitive to proteolytic enzymes, suggesting a lipopetidemolecule (Motta et al. 2007). The objective of this work wasthe description of a new Bacillus sp. strain P34 and to pro-vide further characterization of its antibacterial substance.
Materials and methods
Reagents and media
Brain heart infusion (BHI) broth was from Oxoid (Basing-stoke, UK). Trypticase soy broth (TSB) was from Acumedia(Baltimore, USA). Lipase (from Candida rugosa), trypsinand pronase E were from Sigma (St. Louis, USA). All othermedia and reagents were from Merck (Darmstadt, Germany).
Bacterial strains and culture conditions
The producer strain P34 was given by Universidade Federaldo Amazonas (Manaus, Brazil). The organism was isolatedfrom the intestinal contents of the teleost Wsh Piau-com-pinta (Leporinus sp.) of Amazon basin, at central Amazo-nia, near Manaus, Brazil (3°06�S, 60°01�W).
The indicator strains used in the study were from ATCC(American Type Culture Collection, Rockville, USA),NCTC (National Collection of Type Culture, Colendale,UK) and our own culture collection (UFRGS, Porto Alegre,Brazil) and were kept frozen at ¡21°C in BHI containing20% (v/v) glycerol.
Taxonomical studies
Phenotypic characterization of the strain P34 included mor-phological, cultural, physiological, biochemical and antibiotic
susceptibility features, listed in Table 1. All test procedureswere carried out as described elsewhere (Claus and Berke-ley 1986; MacFaddin 2000). B. subtilis ATCC 6633 and B.licheniformis ATCC 14580 were used as reference strains.Additionally, an API 50CHB kit was used and the data wassubmitted to automated interpretation using the APILABPlus software (BioMérieux, Marcy-l’Etoile, France).
The sequence of 16S rDNA was obtained after genomicDNA extraction, PCR ampliWcation and sequencing basedon previous work (Bastos et al. 2000). The bacterial 16SrRNA sequencing primers were fD1 (5�-AGAGTTTGATCCTGGCTCAG-3�) and rD1 (5�-AAGGAGGTGATCC
Table 1 Phenotypic characteristics of strain P34
Character Result
Cells size 2.9 £ 0.8 �m
Spores Elliptical at subterminal position
Gram-stain Positive
Motility Positive
Esculin Positive
Casein hydrolysis Positive
Starch hydrolysis Positive
Tyrosine Negative
Catalase Positive
Lecithinase Negative
Acetoin Positive
Indole Negative
Citrate Positive
Gelatin liquefaction Positive
Nitrate reduction Positive
Anaerobic growth Negative
Growth in NaCl (%, w/v)
5 Positive
7 Positive
10 Positive
Growth at 50°C Positive
Growth at pH 5.7 Positive
Fermentation
Glucose Positive
Arabinose Positive
Xylose Negative
Manitol Positive
Gas production from glucose Negative
Susceptibility
Penicillin Sensitive
Streptomycin Sensitive
Vancomicin Sensitive
Ceftibuten Resistant
Novobiocin Resistant
CiproXoxacin Resistant
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Arch Microbiol (2007) 188:367–375 369
AGCC-3�); 341–357f (5�-CCTACGGGAGGCAGCAG-3�)and 357–341r (5�-CTGCTGCCTCCCGTAGG-3�); 685–704f (5�-GTAGSGGTGAAATSCGTAGA-3�) and 704–685r(5�-CTACGSATTTCACCSCTAC-3�); 1099–1114f (5�-GCAACGAGCGCAACCC-3�) and 1114–1099r (5�-GGGTTGCGCTCGTTGC-3�). The DNA was ampliWed using aGeneamp PCR System 2400 (Perkin Elmer, Norwalk, USA)by denaturation at 96°C (3 min), 30 cycles consisting of94°C (1 min), 55°C (30 s) and 72°C (2 min), and a Wnalextension step at 72°C (7 min). The PCR-ampliWed 16SrDNA was sequenced by the ABI Prism 377 DNASequencer (Perkin Elmer) based on Xuorescent-labeleddideoxynucleotide terminators. The 1,522-bp sequence wassubmitted to Genbank (accession number AY962472). TheBLAST algorithm was used to search for homologoussequences in Genbank. The phylogenetic tree was inferredfrom Jukes-Cantor distances using the neighbor-joiningmethod (software MEGA3, Kumar et al. 2004). The branch-ing pattern was checked by 1,000 bootstrap replicates.
Transmission electron microscopy
Cells of strain P34 were harvested from BHI agar platesafter 24 h of incubation at 37°C. The cells were Wxed with2.5% (v/v) glutaraldehyde, 2% (v/v) formaldehyde in0.12 mol l¡1 phosphate buVer for 10 days and then pos-Wxed in 2% (w/v) osmium tetroxide in the same buVer for45 min before dehydration. Dehydration was done in agraded acetone series (30–100%) and embeeding in Aral-dite-Durcupan for 72 h at 60°C. Thin sections were pre-pared with a Leica Ultracul UCT ultramicrotome (Leica,Benshein, Germany), mounted on grids, covered with col-lodium Wlm, and poststained with 2% (w/v) uranyl acetatein Reynold’s lead citrate. All preparations were observedwith a Philips EM 208-5 transmission electron micro-scope (Philips Electronic Instruments Inc., Mahwah,USA) operating at 100 kV.
Production of antimicrobial substance
For the production of antibacterial substance, the strain P34was grown in 100 ml BHI-medium at 30°C in a rotaryshaker at 180 cycles min¡1 for desired times. Determina-tion of the number of viable cells (CFU ml¡1) was carriedout as described elsewhere (Motta and Brandelli 2002).After cultivation for 24 h, the cells were harvested by cen-trifugation at 10,000g for 15 min and the culture superna-tant was sterilized by Wltration with 0.22 �m membranes(Millipore, Bedford, USA). The Wltrate was precipitatedwith ammonium sulfate at 20% saturation. The precipitatewas dissolved in 10 mM phosphate buVer pH 7.0. Thissolution was further puriWed by gel Wltration chromatogra-phy on a Sephadex G-100 column. Fractions positive for
antimicrobial activity were pooled and applied to a columnof DEAE-Sepharose, eluted with the same buVer followedby a gradient from 0 to 1.5 M NaCl. The active peaks weredialyzed and rechromatographed according to the sameprocess. Purity was checked by cappilary zone electropho-resis, performed as described elsewhere (Bastiani et al.2002), and using a 60 cm £ 50 �m capillary. Samples of5 ml were run in 50 mM borate buVer pH 9.2, and detectedby laser Xuorescence.
Antimicrobial activity assay
Antimicrobial activity was determined essentially asdescribed previously (Motta and Brandelli 2002). An ali-quot of 20 �l of partially puriWed BLIS was applied ondiscs (6 mm) on BHI agar plates previously inoculated witha swab submerged in a indicator strain suspension whichcorresponded to a 0.5 McFarland turbidity standard solu-tion. Plates were incubated at the optimal temperature ofthe test organisms (Table 2) and inhibitory zones were mea-sured after 24 h.
The antimicrobial activity titre was determined by theserial twofold dilution method previously described byMayr-Harting et al. (1972). Activity was deWned as thereciprocal of the dilution after the last serial dilution givingan inhibition zone and expressed as arbitrary unit (AU) permililitre. The AU ml¡1 were determined against L. mono-cytogenes ATCC 7644 as indicator strain.
Chemical stability
Partially purifed BLIS samples were used to determine thesusceptibility in diVerent conditions essentialy as describedpreviously (Cladera-Olivera et al. 2004). Samples (1 ml)were treated at 37°C for 60 min with 2 mg ml¡1 (Wnal con-centration) of trypsin, pronase E and lipase. Samples werethen boiled for 3 min for enzyme inativation.
The antimicrobial activity at diVerent pH values wasestimated by adjusting the pH of samples from pH 3.0 to10.0. To evaluate pH stablitity, the antimicrobial substancewas incubated at pH 3.0–10.0 for 30 min and the pH wasneutralized to 7 before testing for antimicrobial activity.
Chemicals (working concentration in Table 3) wereadded to the antimicrobial substance and the samples wereincubated for 60 min at 37°C before being tested for anti-microbial activity. After treatments with TCA, sampleswere centrifuged at 10,000g for 5 min, pellet was solubi-lized in 10 mM Tris pH 8.0 and the supernatant was neu-tralized to pH 7.0, before testing for antimicrobial activity.Chemicals diluted with 8.75 g l¡1 NaCl were used ascontrols.
After each treatment the samples were tested for antimi-crobial activity againts L. monocytogenes ATCC 7644.
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370 Arch Microbiol (2007) 188:367–375
EVect on L. monocytogenes and B. cereus
Overnight cultures of L. monocytogenes ATCC 7644 andB. cereus 8A were obtained by growing in TSB mediumat 37°C for 18 h. A sample (1%) of those cultures wereinoculated in Erlenmeyer Xasks containing 50 ml TSB and
incubated at 37°C. The growth was checked at 2-h intervalsby O.D. 600 nm and by viable cell counts (CFU ml¡1).
BLIS (Wnal concentration 160 AU ml¡1) was added sep-arately, to culture of L. monocytogenes and B. cereus after6 h of growth and the eVect on turbidity and on the numberof viable cells was determined at 2-h intervals. The colo-nies were counted after 24 h of incubation at 37°C.
Results
Characterization of strain P34
The morphological and physiological characteristics ofthe isolate are summarized in Table 1. Microscopicobservation of the isolate showed a straight rod withendospores. The spores were eliptical, located at subter-minal position. Morphological features were detailed bytransmission electron microscopy, revealing a typicalGram-positive cell envelope proWle (Fig. 1). The cyto-plasmic membrane was surrounded by a thin peptidogly-can layer; an overlaid surface layer was separated frompeptidoglycan by a zone of low contrast. The bacteriumgrew aerobically, was strongly catalase positive, pre-sented variable Gram-stain, and was Gram-positive in theKOH test. Together with additional biochemical tests(Table 1) and the use of an API 50CHB kit, these charac-teristics indicated that the isolate belongs to the genusBacillus (Claus and Berkeley 1986). The analysis with
Table 2 Antimicrobial activity spectrum of BLIS P34
Diameter of the inhibition zone in mm around the disk
Strains of the following microorganisms were not inhibited: Brocho-thrix thermosphacta, Staphylococcus aureus, Staphylococcus epide-rmidis, Staphylococcus intermedius, Streptococus sp., Enterococcusfaecalis, S. Enteritidis, Escherichia coli, Enterobacter aerogenes,Pseudomonas aeruginosa, Pseudomonas sp., Candida sp., C. keWr,C. utilis, Kluyveromices marxianus, Malassezia sp
Indicator organism Temperature (°C)
Inhibition zone (mm)
Gram-positive bacteria
Bacillus cereus (food isolate) 37 9.8
B. cereus 8A (soil isolate) 37 10.0
B. subtilis (ICBS-1) 37 9.6
Lactobacillus acidophilus ATCC 4356 37 9.8
Brevibacterium linens ATCC 9172 25 9.2
Brevibacterium linens ATCC 9174 25 9.0
Brevibacterium linens ATCC 9175 25 9.2
Brevibacterium linens ATCC 19391 25 9.8Corynebacterium Wmi NCTC 7547 37 9.7
Listeria monocytogenes ATCC 7644 37 12.3
L. innocua (food isolate) 37 11.3
Listeria spp. (clinical isolate) 37 11.0
L. monocytogenes (clinical isolate) 37 13.0
L. monocytogenes 4C 37 13.0
L. monocytogenes 1 7D78/03 37 13.0
L. innocua ATCC 33090 37 11.5
L. innocua 1572 37 12.5
L. ivanovii 5 NCTC 11007 37 11.0
L. seeligeri AC 82/4 37 9.0
L. welshimeri AC 73/2 37 13.0
Rhodococcus sp. 37 13.0
Gram-negative bacteria
Salmonella Gallinarum (clinical isolate)
37 8.5
Erwinia carotovora 413 25 8.2
E. carotovora 416 25 8.2
E. carotovora 325 25 8.7
E. carotovora 365 25 8.2
Aeromonas hydrophila (clinical isolate)
28 8.5
Pasteurella haemolytica (clinical isolate)
37 9.0
P. haemolytica (clinical isolate) 37 9.0
Table 3 EVect of chemical substances on antimicrobial activity usingL. monocytogenes ATCC 7644 as indicator strain
Control, after proteolytic treatment the bacteriocin was boiled for3 min at 100°C for protease inactivation
Treatment Concentration Residual activity (%)
Untreated bacteriocin – 100
Boiled 3 min* – 100
Lipase 2 mg ml¡1 15
Trypsin 2 mg ml¡1 40
Pronase E 2 mg ml¡1 0
Acetone 50% (v/v) 80
Chloroform 50% (v/v) 100
Dimethyl sulfoxide 50% (v/v) 100
Ethanol 50% (v/v) 100
Methanol 50% (v/v) 80
Butanol 50% (v/v) 40
Xylol 50% (v/v) 100
EDTA 10 mM 100
2-mercaptoethanol 10 mM 0
Trichloroacetic acid 100 mg ml¡1 0
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Arch Microbiol (2007) 188:367–375 371
the APILAB Plus software indicated a very good identityto the genus Bacillus.
The phylogenetic analysis conWrmed that the isolatewas a Bacillus sp. and revealed that strain P34 was clos-est to B. infernus (Fig. 2). The P34 sequence shared lowsimilarity with most Bacillus species and showed 91%similarity with B. infernus. The cluster formed by P34and B. infernus was supported by high bootstrap values(Fig. 2).
Production of antimicrobial activity
Bacillus sp. P34 was aerobically incubated in BHI mediumat 30°C. Exponential cell growth reached the stationaryphase after 12 h of cultivation (Fig. 3). Remarkably, anti-bacterial activity can be observed in the exponential growthphase (6 h), with maximal values in the stationary phase
(24–30 h). It was observed that pH values were nearlyconstant (pH = 7.0–7.5) during cultivation.
The antimicrobial substance obtained at 24 h of cultiva-tion, was then puriWed from the culture supernatant byammonium sulfate precipitation and liquid chromatogra-phy. The antimicrobial activity eluted in the void volume ofthe Sephadex G-100 column, separated of the main bulk ofprotein. This column was also eluted with buVer containing1.5 M NaCl, and the activity was detected within theincluded volume of the column (not shown). Further puriW-cation by ion exchange chromatography yielded a singlepeak containing the antimicrobial activity. A single compo-nent was observed by capillary electrophoresis, conWrmingthe homogeneity of the puriWed molecule. As a single anti-microbial substance was detected, subsequent experimentswere carried out with the partially puriWed fraction from gelWltration chromatography.
Inhibitory spectrum
The antimicrobial substance was active against Gram-posi-tive and Gram-negative bacteria, including important path-ogenic and spoilage microorganisms. The results are shownin Table 2. The inhibitory activity was observed on L. mon-ocytogenes, L. innocua, Corynebacterium Wmi, B. cereus,B. subtilis, Erwinia carotovora, Aeromonas hydrophila,Pasteurella haemolytica, among other. L. monocytogenesATCC 7644 was used as indicator strain in subsequentexperiments.Fig. 4
Chemical stability
The antimicrobial substance was tested for sensitivity toenzymes and residual activity was measured by agar disc
Fig. 1 Thin sections of cells of strain P34, showing round to spore lo-cated subterminally within sporangium. The cell envelope shows mul-tiple layers, where the outermost layer exhibits the regularly arrangedstructure of the S layer. Bar 300 nm
Fig. 2 Phylogenetic position of strain P34 within the genus Bacillus. The branching pattern was generated by the neighbour-joining method. The number of each branch indicate the boot-strap values. Bar 0.1 Jukes-Can-tor distance
Bacillus subterraneus (AY672638)
Bacillus firmus (AY833571)
Bacillus lentus (AB021189)
Bacillus subtilis (X60646)
Bacillus amyloliquefaciens (X60605)
Bacillus licheniformis (X68416)
Bacillus coagulans (D16267)
Bacillus thermocloacae (Z26939)
Bacillus thermosphaericus (X90640)
Bacillus thermoleovorans (Z26923)
Bacillus stearothermophilus (AB021196)
Bacillus thermoglucosidasius (AB021197)|
Bacillus acidocaldarius (X60742)
Bacillus infernus (U20385)
P34
100
99
99
92
86
81
74
54
54
41
50
100
0.1
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diVusion assay against L. monocytogenes ATCC 7644. Thesubstance was sensitive to lipase, trypsin and pronase E atthe concentration of 2 mg ml¡1 (Table 3).
The eVect of several chemicals on the antimicrobialactivity was evaluated. The substance lost its activity aftertreatment with trichloroacetic acid (TCA) and 2-mercapto-ethanol (Table 3). When treated with organic solvents andother chemicals, the antimicrobial activity was onlyaVected by butanol, and in lesser extent by acetone andmethanol (Table 3).
The antimicrobial substance was stable in all pH tested(3.0–10.0), remaining 100% its initial activity. When theactivity was tested within this pH range, at least 70% ofmaximum activity, observed at pH 6.0–8.0, was observed.
Considering the properties of the inhibitory substanceproduced by Bacillus sp. strain P34, it was characterized asa bacteriocin-like compound.
EVect on L. monocytogenes and B. cereus
The eVects of the BLIS on the growth of L. monocytogenesand B. cereus are shown in Fig. 4. The addition of BLIS(160 AU ml¡1) to cells suspensions of L. monocytogenes orB. cereus at the exponential growth phase results in a diVer-ence in viable counts related to the controls. The addition ofthe antimicrobial substance inhibited the growth of the indi-cator strains resulting in a decrease in the number of viablecells and in optical density over a period of 24 h (Fig. 4).This indicated that BLIS has a bactericidal and bacteriolyticeVect.
Discussion
A bacterium producing a BLIS was isolated from the intes-tinal contents of Leporinus sp., a teleost Wsh of Amazonbasin, and was identiWed as Bacillus sp. by biochemicalproWling and 16S rDNA sequencing. From the sequenceanalysis of the 16S rDNA gene, strain P34 was found to beclustered with the B. infernus, although an important diVer-ence in sequence was observed. In addition, B. infernusthrives in heat and anaerobiosis (Boone et al. 1995).Because these characteristics are not in agreement withthose of strain P34, this species can be assigned to thegenus level as Bacillus sp. These data suggest that our iso-late is a new Bacillus species (Stackebrandt and Goebel1994; Palys et al. 1997; Goto et al. 2000). Considering itwas isolated from a Wsh of Brazilian Amazon basin, wepropose this bacterium be classiWed in the genus Bacillus as“B. amazonensis”.
The antimicrobial substance was shown to be broadlyactive, which is also typical of Gram-positive BLIS andparticularly of antimicrobial peptides produced by Bacillus
Fig. 3 Production of antimicrobial activity by strain P34. Bacterialgrowth (circles) and antibacterial activity (squares) were monitoredduring growth in BHI at 30°C. Each point represents the mean of threeindependent experiments. The indicator strain was Listeria monocyt-ogenes ATCC 7644
Time (h)
0 10 20 30 40 50
mn 006 .D.
O
0
1
2
lm
UA
1-
0
400
800
1200
Fig. 4 EVect of BLIS on growth of B. cereus (a) and L. monocytoge-nes (b). Turbidity (black symbols) and viability (open symbols) weremonitored in control (circles) and treated (squares) cells. Each pointrepresents the mean of three independent experiments
Time (h)
0 5 10 15 20 25
mn 006 .D.
O
0,0
0,5
1,0
1,5
2,0
gol01
lm
UF
C 1-
0
2
4
6
8
10
Time (h)
0 5 10 15 20 25
mn 006 .D.
O
0,0
0,5
1,0
1,5
gol01
lm
UF
C 1-
0
2
4
6
8
10
A
B
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species (Jack et al. 1995; Hyronimus et al. 1998; Bizani andBrandelli 2002; Risoen et al. 2004). C. Wmi NCTC 7547,described as being susceptible to all bacteriocins tested(Oliveira et al. 1998), was also sensitive to the BLIS pro-duced by Bacillus sp. P34. The antimicrobial substance wasable to inhibit the growth of L. monocytogenes, a veryimportant property in food safety. A. hydrophila, an impor-tant pathogen linked to seafood and water outbreaks (Tsaiand Chen 1996), was also inhibited. Therefore, this novelBLIS may represent a relevant alternative against severalfood pathogenic and spoilage microorganisms.
The production of antimicrobial activity stated duringthe exponential growth phase, reaching maximum values atstationary phase. Production of antimicrobial peptides bystrains of Bacillus is suggested to be under complex geneticregulation (Marahiel et al. 1993; Duitman et al. 1999). Ithas been observed that modiWcation of the culture condi-tions, like nitrogen source and pH, may induce the produc-tion of diVerent antimicrobial peptides. A single strain canproduce diVerent antimicrobial peptides simultaneously orat least at diVerent time intervals or growth conditions(Duitman et al. 1999). Decrease of antimicrobial activity atthe late stationary phase could be associated to degradationby extracellular proteases, which are often produced byBacillus spp. (Bizani and Brandelli 2002). However, mostof the known bacteriocins are highly stable against the pro-teases of producer strain. The activity of linocin M18, abacteriocin that forms large proteinaceous aggregates,diminished rapidly after 1–2 days at room temperature,even in the presence of protease inhibitors (Valdes-Stauberand Scherer 1994).
Bacteria can produce a variety of inhibitory substances.In this case, organic acids can be ruled out, since the pH inthe growth medium was always in the range of 7.0–7.5 dur-ing cultivation in BHI. The antimicrobial activity was sen-sitive to the enzymes tested, with complete inactivation bythe broad range protease pronase E, indicating its proteina-ceous nature. In addition, BLIS sensitivity to lipase maysuggest a lipopeptide structure, in agreement to previousresults of infrared spectroscopy (Motta et al. 2007). A bac-teriocin produced by B. licheniformis, Lichenin A, wascompletely inactivated by proteinase K treatment but wasresistant to trypsin (Pattnaik et al. 2001). Enzymes such asproteinase K and pronase E were shown to eliminate thuri-cin 439 activity, indicating a bacteriocin-like inhibitorycompound (Ahern et al. 2003). The fact that the antimicro-bial activity was completely lost by only few enzymes andwas inactivated by 2-mercaptoethanol may suggest that theBLIS have intamolecular disulWde bonds. This agrees withthe fact that the inhibitory compound was relatively heatstable and shows stability within the pH range of 3.0–10.0.A BLIS from B. amyloliquefaciens strain I3 was recentlycharacterized (Lisboa et al. 2006), showing diVerent pH
stability and increased resistance to proteases when com-pared with P34.
The BLIS appeared as a single band with a molecularmass of about 6 kDa, and shown a molecular mass of1,456 Da by mass spectroscopy (Motta et al. 2007). How-ever, the antimicrobial activity eluted in the void volume ofthe Sephadex G-100 column. This indicates that nativeBLIS forms aggregates of high molecular masses(>150 kDa). This behavior was similar to that observed forthe bacteriocin linocin M18 (Valdes-Stauber and Scherer1994). Some bacteriocin molecules present a substantialportion of hydrophobic residues and their association intolarge aggregates is possibly because of the highly hydro-phobic nature of the peptides.
The decline in the number of living cells of L. monocyt-ogenes and B. cereus after the addition of BLIS suggest thatthe antimicrobial eVect was bactericidal. The decrease inO.D. readings indicated that cells of indicator strains werelysed. It has been suggested that the antimicrobial eVect canbe dependent on the assay conditions, such as the amountand purity of bacteriocin, culture media, indicator strainand its cellular concentration (Motta and Brandelli 2002).The BLIS identiWed in this work showed bactericidal andbacteriolytic eVect on L. monocytogenes and B. cereus at160 AU ml¡1.
Bacteriocins may play a defensive role to hinder theinvasion of ecosystem of other strains or species into anoccupied niche (Riley and Wertz 2002). Antibacterial sub-stances produced by diVerent bacteria seem to play animportant role in the bacterial antagonism in aquatic eco-systems (Dopazo et al. 1988). In addition, it has been foundthat intestinal bacteria from both freshwater and marineWshes show an inhibitory eVect on Wsh pathogenic bacteria(Olsson et al. 1992; Sugita et al. 1996). These include anti-microbial substances produced by Bacillus strains isolatedfrom Wsh intestines (Sugita et al. 1998; Ghosh et al. 2003).A similar role could be assigned to the strain P34, where itsBLIS may help to avoid pathogen colonization of Wsh intes-tines. The broad inhibitory spectrum of strain P34 mayindicate an ecological advantage, since it would be capableto inhibit several competing bacteria.
While many studies on BLIS have shown their impor-tance as food preservatives, few attention have beenaddressed to their application as antimicrobials in clinicalstudies. Because bacteriocin treatment is potentially eVectiveand non-toxic to human and animals, it has been already pro-posed as an alternative for disease control (Oliveira et al.1998; Twomey et al. 2000). The BLIS produced by strainP34 may represent an antimicrobial substance with potentialapplication in the prevention and treatment of SalmonellaGallinarum, which causes severe systemic disease in domes-tic poultry (Johnson et al. 1977). In this regard, the lantibioticmersacidin produced by B. subtilis has shown promising
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374 Arch Microbiol (2007) 188:367–375
applications particularly against methicillin-resistant staphy-lococci (Bierbaum et al. 1995). The rapid rise and spread ofmulti-resistant bacterial pathogens have forced the consider-ation of alternative methods of combating infections. Forexample, several strains of L. monocytogenes have acquiredresistance to conventional bacteriocins (Rasch and Knochel1998; van Schaik et al. 1999). Thus, there is a need for newsubstances that exhibit eYcient antimicrobial activity againstsuch strains. Given the diversity of bacteriocins produced innature, they can be considered as an alternative to combatinfections against speciWc pathogens (Neu 1992; Riley andWertz 2002). Therefore, research for new products with anti-microbial activity is a very important Weld. The identiWcationand chemical characterization of bacteriocins produced byBacillus spp., and exploration of their potential use in thecontrol of pathogenic and spoilage microorganisms addressesthis subject.
Acknowledgments Authors thank Dr. Spartaco AstolW-Filho fromUniversidade Federal do Amazonas for kindly provide the bacterialstrain P34, Centro de Microscopia Eletronica of UFRGS and ULBRAfor technical support in electron microscopy. This work received Wnan-cial support from CNPq and CAPES, Brazil.
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